Mercurial > repos > bebatut > metaphlan2
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planemo upload for repository https://github.com/ASaiM/galaxytools/tree/master/tools/sortmerna/ commit 90c51a29d5aaab3f8dea67ac12098dc386e23b4e-dirty
| author | bebatut |
|---|---|
| date | Thu, 05 Nov 2015 09:03:13 -0500 |
| parents | 31dd7ace2be4 |
| children | 615111232408 |
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<tool id="metaphlan2" name="MetaPhlAn2" version="0.1.0"> <description>to profile the composition of microbial communities</description> <requirements> <requirement type="package" version="2.2.5">bowtie2</requirement> <requirement type="package" version="2.0">metaphlan2</requirement> </requirements> <stdio> <exit_code range="1:" /> </stdio> <version_command> <![CDATA[ python \${METAPHLAN2_DIR}/metaphlan.py -v ]]> </version_command> <command> <![CDATA[ python \${METAPHLAN2_DIR}/metaphlan.py $input_file -o $output_file --input_type ${input_file.datatype.file_ext} --mpa_pkl \${METAPHLAN2_DIR}/db_v20/mpa_v20_m200.pkl --bowtie2db \${METAPHLAN2_DIR}/db_v20/mpa_v20_m200 $bowtie2_output #if $bowtie2_output == '' --bowtie2out $bowtie2_output #end if -t $analysis_type$analysis_type_select #if $analysis_type.analysis_type_select == "rel_ab" --tax_lev $analysis_type.taxonomic_level #else if $analysis_type.analysis_type_select == "marker_ab_table" --nreads $analysis_type.nreads #else if $analysis_type.analysis_type_select == "marker_pres_table" --pres_th $analysis_type.pres_th #end if --min_cu_len $min_cu_len --min_alignment_len $min_alignment_len $ignore_viruses $ignore_eukaryotes $ignore_bacteria $ignore_archaea --stat_q $stat_q #if $sam_output -s $sam_output_file #end if #if $biom_output -biom $biom_output_file #end if ]]> </command> <inputs> <param name="input_file" type="data" format="fastq,fasta,sam,bowtie2out" label="Input file" help=""/> <conditional name="analysis_type"> <param name="analysis_type_select" type="select" label="Type of analysis to perform"> <option value="rel_ab" selected="true">Profiling a metagenomes in terms of relative abundances</option> <option value="rel_ab_w_read_stats">Profiling a metagenomes in terms of relative abundances and estimate the number of reads comming from each clade</option> <option value="reads_map">Mapping from reads to clades (only reads hitting a marker)</option> <option value="clade_profiles">Normalized marker counts for clades with at least a non-null marker</option> <option value="marker_ab_table">Normalized marker counts (only when > 0.0 and normalized by metagenome size if --nreads is specified)</option> <option value="marker_pres_table">List of markers present in the sample (threshold at 1.0 if not differently specified with --pres_th</option> </param> <when value="rel_ab"> <param name="taxonomic_level" type="select" label="Taxonomic level for the relative abundance output"> <option value="a" selected="true">All taxonomic levels</option> <option value="k">Kingdoms (Bacteria and Archaea) only</option> <option value="p">Phyla only</option> <option value="c">Classes only</option> <option value="o">Orders only</option> <option value="f">Families only</option> <option value="g">Genera only</option> <option value="s">Species only</option> </param> </when> <when value="marker_ab_table"> <param name="nreads" type="integer" value="0" label="Total number of reads in the original metagenome" help="It is used for normalizing the length-normalized counts with the metagenome size as well. No normalization applied if the value is not specified"/> </when> <when value="marker_pres_table"> <param name="pres_th" type="integer" value="0" label=" Threshold for calling a marker present" help=""/> </when> </conditional> <param name="min_cu_len" type="integer" value="2000" label="Minimum total nucleotide length for the markers in a clade for estimating the abundance without considering sub-clade abundances" help=""/> <param name="min_alignment_len" type="integer" value="0" label="Sam records for aligned reads with the longest subalignment length smaller than this threshold will be discarded." help=""/> <param name="ignore_viruses" type='boolean' checked="true" truevalue='' falsevalue='--ignore_viruses' label="Profile viral organisms?" help="" /> <param name="ignore_eukaryotes" type='boolean' checked="true" truevalue='' falsevalue='--ignore_eukaryotes' label="Profile eukaryotic organisms?" help="" /> <param name="ignore_bacteria" type='boolean' checked="true" truevalue='' falsevalue='--ignore_bacteria' label="Profile bacteria organisms?" help="" /> <param name="ignore_archaea" type='boolean' checked="true" truevalue='' falsevalue='--ignore_archaea' label="Profile archea organisms?" help="" /> <param name="stat_q" type="float" value="0.1" label="Quantile value for the robust average" help=""/> <param name="bowtie2_output" type='boolean' checked="true" truevalue="" falsevalue='--no_map' label="Store the output of BowTie2?" help="" /> <param name="sam_output" type='boolean' label="Output a sam file?" help="" /> <param name="biom_output" type='boolean' label="Output a biom file?" help="" /> </inputs> <outputs> <data format="txt" name="output_file" metadata="input_sequence_file" label="Profile of communities on ${on_string} (MetaPhlAn)" /> <data format="bowtie2" name="bowtie2_output_file" metadata="input_sequence_file" label="Bowtie2 output on ${on_string} (MetaPhlAn)"> <filter>bowtie2_output != '--no_map' </filter> </data> <data format="sam" name="sam_output_file" metadata="input_sequence_file" label="Sam output on ${on_string} (MetaPhlAn)"> <filter>sam_output</filter> </data> <data format="biom" name="biom_output_file" metadata="input_sequence_file" label="Biom output on ${on_string} (MetaPhlAn)"> <filter>biom_output</filter> </data> </outputs> <tests> <test> <param name="input_file" value="input_sequences.fastq"/> <param name="analysis_type_select" value="rel_ab" /> <param name="taxonomic_level" value="a" /> <param name="min_cu_len" value="2000" /> <param name="min_alignment_len" value="0" /> <param name="ignore_viruses" value="" /> <param name="ignore_eukaryotes" value="" /> <param name="ignore_bacteria" value="" /> <param name="ignore_archaea" value="" /> <param name="stat_q" value="0.1" /> <param name="bowtie2_output" value='--no_map' /> <param name="sam_output" value='False' /> <param name="biom_output" value='False' /> <output name="output_file" file="profiled_metagenome.txt"/> </test> </tests> <help><![CDATA[ **What it does** MetaPhlAn is a computational tool for profiling the composition of microbial communities (Bacteria, Archaea, Eukaryotes and Viruses) from metagenomic shotgun sequencing data with species level resolution .. _MetaPhlAn2 user manual: https://bitbucket.org/biobakery/metaphlan2 ----- **Input** Metaphlan2 takes as input a sequence file in fasta, fastq, a BowTie2 produced SAM file or an intermediary mapping file of the metagenome generated by a previous MetaPhlAn ----- **Parameters** Several parameters can modulate the MetaPhlAn execution * Mapping arguments * Test to avoid saving the output of BowTie2 * Post-mapping arguments * Taxonomic level for the relative abundance output * Minimum total nucleotide length for the markers in a clade for estimating the abundance without considering sub-clade abundances * Sam records for aligned reads with the longest subalignment length smaller than this threshold will be discarded * Tests to avoid profiling of virus, eukaryotes, bacteria and/or archea * Quantile value * Additional analysis types and arguments * Type of analyse to perform and some parameters for specific analysis type ----- **Outputs** The main output file is a tab-separated output file of the predicted taxon relative abundances. Given the choosen parameters, other output files can be: * a sam output file * a biom output fime * a BowTie2 output file ]]></help> <citations> <citation type="doi">10.1038/nmeth.3589</citation> </citations> </tool>